Quantitative analysis of α 1 (I) procollagen transcripts in vivo by competitive polymerase chain reaction

1996 
Abstract Due to the limited amount of RNA obtainable from punch biopsies, few data exist on the human α 1 (I) procollagen mRNA steady state level in vivo . Therefore, we established a competitive PCR method to quantitate this mRNA in human biopsies. In our approach, the target template and the standard share the same sequence except for a 69 bp deletion, thus competing for the same primer pair and subsequently amplifying at the same rate. Titration of a competitor DNA dilution series against an unknown cDNA sample then allows quantitation of the separated and nonradioactively detected PCR products after densitometrical analysis. Almost identical results were obtained by quantitation of the same total RNA by competitive PCR as well as Northern blot analysis.
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